The covalent structure of a human γG ... - ACS Publications

of the Cyanogen Bromide Fragments*. Myron J. Waxdal, William H. Konigsberg, and Gerald M. Edelman abstract: The arrangement of ten pairs of fragments...
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The Covalent Structure of a Human yG-Immunoglobulin. 111.Arrangement of the Cyanogen Bromide Fragments* Myron J. Waxdal, William H. Konigsberg, and Gerald M. Edelman

The arrangement of ten pairs of fragments produced by the CNBr cleavage of a human yG-immunoglobulin (Eu) has been determined. The three light-chain fragments were ordered on the basis of their NH,- and COOH-terminal amino acid residues. This order was consistent with the amino acid sequence of tryptic peptides which overlapped the sites of CNBr

ABSTRACT:

w

e have reported (Waxdal et al., 1968) the isolation, composition, and location of ten unique CNBr fragments from a human yG-immunoglobulin. I n the present paper we describe experiments which have enabled us to deduce the arrangement of regions corresponding to the CNBr fragments in the intact light and heavy chains. The light chains produced only three fragments after CNBr treatment, and the order of these fragments was unambiguously fixed once the NHn- and COOHterminal CNBr fragments were identified. These assignments were consistent with the sequences of methioninecontaining peptides (overlap peptides) from a tryptic digest of the light chain. The arrangement of the CNBr fragments of the heavy chain was deduced by isolation and partial sequence determination of overlap peptides from tryptic digests of the Fd(t)l and Fc(t) portions of the heavy chain. Materials and Methods The purification of Eu, subsequent cleavage by CNBr, and isolation of the fragments have previously been described in detail (Edelman et al., 1968; Waxdal et ul., 1968). Tryptic Digesrion. Trypsin treated with L-l-tosylamino-2-phenylethyl chloromethyl ketone was obtained

* From The Rockefeller University, New York, New York, and the Department of Biochemistry, Yale University, New Haven, Connecticut (W. H. K.), Receiwd January 8, 1968. This work was supported in part by grants from the National Science Foundation (GB-6546 and GB-6655) and the U. S. Public Health Service (AM 04256-08 and GM 12607-03). Part of this work was presented at the 32nd Cold Spring Harbor Symposium on Quantitative Biology, 1967 (Waxdal et a/., 1967), the Nobel Symposium 3 on y-Globulins, Sodergarn, Sweden, 1967 (Edelman, 1967), and the 7th International Congress of Biochemistry, Tokyo, 1967 (Edelman et al., 1967). 'Abbreviations used that are not listed in Biochemistry 5, 1445 (19661, are: Fab(t), Fc(t), Fd(t), tryptic fragments corresponding to Fab, Fc, and Fd (World Health Organization, 1964); dansyl, 1-dimethylaminonaphthalene-5-sulfonyl; Asx, aspartic acid or asparagine; Glx, glutamic acid or glutamine.

cleavage. The seven heavy-chain fragments were placed in order by analysis of tryptic overlap peptides isolated from the Fd(t) and Fc(t) portions of the heavy chains. These assignments provide proof for current models of human yG-immunoglobulins and allow formulation of a more detailed model.

from Calbiochem (Los Angeles, Calif.). The CNBr fragments, light chain, and the Fd(t) and Fc(t) portions of the heavy chain were digested with trypsin for 4 hr (protein concentration, 1 ; trypsin concentration, 0.01%). The temperature was maintained at 37" and the p H at 7.8 by the use of a pH-Stat. After digestion the pH was lowered to 3.1 and the solution was lyophilized. Zon-Exchange Chromatography. Peptides were fractionated by ion-exchange chromatography on polystyrene resins substituted with sulfonic or trimethylammonium groups (Bio-Rad Laboratories, Richmond, Calif.) using pyridine acetate buffers (cf. Schroeder e f ul., 1962). The effluent stream was split and a portion continuously monitored before and after hydrolysis in NaOH using a modification of the method described by Catravas (1964). AG-50x4. The resin (30-35-p particles) was packed into a 185 X 0.9 cm column and was eluted at 60" at a flow rate of 30 mljhr maintained with a pump (miniPump, Milton Roy, Philadelphia, Pa.). The back pressure under these conditions rose from 80 t o 150 psi during the elution. Two linear gradients were used with this resin; in both cases 350 ml of each buffer was placed in separate flasks serially connected by siphons. Flask A was connected to the eluent pump. Gradient I had (1) flask A, 0.2 M pyridine adjusted to p H 3.1 with acetic acid; and (2) flask B, 2.0 M pyridine adjusted to pH 5.5 with acetic acid. Gradient I1 had ( 1 ) flask A, 0.05 hi pyridine adjusted to pH 3.1 with acetic acid; (2) flask B, 0.20 M pyridine adjusted to pH 3.1 with acetic acid; and (3) flask C , 2.00 M pyridine adjusted to pH 5.5 with acetic acid. I n some experiments the columns were washed overnight with the p H 5.5 buffer after the gradient was completed in order to elute tightly bound peptides. The resin was regenerated in the column by washing with the initial buffer until the p H and ionic strength of the effluent matched that of the incoming buffer. AG-50x12. The resin (2-19-p particles) was packed into a 60 x 0.9 cm column. The conditions of chroma-

C O V A L E NT

S T R U C T IJ R E

0F

G

-IMM

1967

U N0G L 0B U L I N

n 1 0 C 11 LO-1 Leu-Leu-Met-Tyr-Lys LO-la LO-lb Leu-Leu-Hsr Tyr-Lys

Overlap tryptic peptides containing methionine CNBr fragments of overlap peptides COOH- and "%-terminal residues of CNBr fragments from the light chains

Asx-.

L1

. .-Hsr

Tyr----..---

hl I S T R Y

LO-2 Met-Phe-GIy-Glx-GIy-Thr-Lys LO-2a LO-2b Hsr Phe-Gly-Glx-Gly-Thr-Lys

L?

Hsr Phe--...--

LI

----CYS

1 : Ordering of the CNBr fragments (L,, Lp, and L3) of the light chain by comparison of their terminal amino acid residues with the amino acid sequence of tryptic overlap peptides LO-1 and LO-2. FIGURE

tography were the same as those for AG-50x4 except that the back pressure ranged from 200 to 400 psi. AG-ZX2. The resin (-400 mesh) was packed into a 50 x 0.9 cm column. Elution was performed at a flow rate of 90 ml/hr with back pressure less than 25 psi. The columns were eluted at room temperature with a linear gradient from 0.1 M pyridine adjusted to pH 6.5 with acetic acid to 2.0 M acetic acid. An equal amount (350 ml) of each buffer was used to make gradient 111. At the end of the gradient the resin was washed with 25% acetic acid and reequilibrated with the initial buffer. IdentiJicat ion of Methionine-Contuining Peptides. Portions of the pooled ninhydrin-positive material obtained by ion-exchange chromatography were spotted onto Whatman No. 3MM paper and stained with platinic chloride (Easley, 1965). Material which gave a positive stain was subjected to amino acid analysis using a Beckman 120C amino acid analyzer with minor modifications (Edelman et al., 1968). CNBr Cleacage of Peptides. The overlap peptides were dissolved in 70% formic acid (0.5 pmole of peptide/ml) and CNBr ( 5 mg/ml) was added. After 4 hr at room temperature the reaction was stopped by the addition of ten volumes of HaO, and the preparation was lyophilized. Amino Acid Sequence. Edman degradations were per-

I: NHn- and COOH-Terminal Amino Acid Residues of the CNBr Fragments and Chains of Eu:

TABLE

"2-

Fragment

Terminal Amino Acid

Light Chain L1 Lf La

Asx Asx TYr Phe

COOHTerminal Amino Acid CMCys Hsr Hsr CMCys

Blocked Blocked G~Y Phe Glx Ile Thr His

1968

WAXDAL,

KONIGSBERG,

A N D

EDELMAN

Results The terminal amino acid residues of the CNBr fragments and the light and heavy chains are presented in Table I. The compositions of the isolated tryptic peptides from the heavy and light chains which contained methionine (overlap peptides) are presented in Table 11. Order of the Light-Chain CNBr Fragments. The order of the CNBr fragments of the light chain (L1,L2,and L3) could be deduced from a knowledge of the termini of the light chain and of the fragments themselves. As shown in the preceding communication (Waxdal et a/., 1968), CNBr fragment L1 contained a n "*-terminal aspartic acid or asparagine as did the intact light chain (Table I). Because no other major light-chain fragment yielded this end group, LI was placed as the NH,-terminal CNBr fragment. The COOH terminus of both the light chain and Lpwas found to be CM-cysteine (Table I). The presence of a half-cystine residue has previously been reported at the COOH terminus of type K Bence-Jones proteins by a number of authors (Hilschmann and Craig, 1965; Milstein, 1965; Titani et a/., 1965). The CM-cysteine residue was produced by reduction and alkylation of the light-chain-heavy-chain disulfide bond during the preparation of these chains from the intact immunoglobulin (Gall et a/., 1968). The remaining CNBr fragment from the light chain, LL, must occupy the position between L1 and La, and the order is L1-LsL3.

GlY Hsr Hsr Hsr Hsr Hsr Hsr G~Y

From Waxdal et a/. (1968) and Edelman et ul. (1968). fb

formed by a modification of the procedure of Konigsberg and Hill (1962). The new NH2-terminal residue exposed after each cycle of the Edman degradation was identified by dansylation (Gray, 1967) followed by acid hydrolysis and thin-layer chromatography of the dansylamino acid o n polyamide resin plates (Woods and Wang, 1967). An extensive description of this technique is given in a subsequent paper in this series (Cunningham et al., 1968). The NH2-terminalamino acid residues of the CNBr fragments and of light and heavy chains were also determined by this technique.

T o substantiate this conclusion, the light chain was fully reduced, alkylated, and digested with trypsin. Two tryptic peptides which contained methionine (overlap peptides LO-1 and LO-2) were isolated by chromatography on AG50X4 using gradient I1 (Cunningham et al., 1968); their amino acid compositions are presented in Table 11. The amino acid sequences of these peptides have been determined (Cunningham et al., 1968) and are presented in Figure 1 along with the terminal amino acids of the CNBr fragments of the light chain. The peptide LO-1 overlaps the COOH-terminal portion of

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TABLE 11:

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M A Y

Amino Acid Composition of Methionine-Containing Tryptic Peptides from Eu Light and Heavy Chains: ___~

.________

LO-1 ~.

~

LO-2

~~

HO-1

HO-2

~____~_______~

1. o

~~

1. o

-

HO-3 ~~

~

~

~

HO-4 ~

1 .o 0.9 0.4 2.1 1.6 2.9 1.8 0.4 0.2 0.2 1. o

LYS Arg ASP Thr Ser Glu Pro GIY Ala Val Met Ile Leu TYr Phe

0.9

Total residues

5

7

24

20

7

13

20

16

55

10

30

206

% yield

1. o 1.1 1.9

1.1 2.1 0.9

0.9

1. o

1 .o 2.2 3.8 3.2 2.3

1.o 4.2 4.0 4.7 1.9 0.7 1.9 0.7 1 .o 1. o 1.1

0.8 0.8 0.9 1.1

2.0 1.3 0.7 0.9 1.9 0.7

0.9 1.0 1.1

1.2

Values are reported as residues per mole. Amino acid contamination at less than 0.1 mole/mole of peptide is not reported. The values are from single 20-hr hydrolysates and have not been corrected for destruction of threonine and serine nor for incomplete hydrolysis of valine and isoleucine. * After first purification. '1

CNBr fragment L1 and the NH?-terminal portion of LB. This assignment was made because tyrosine followed methionine in the overlap peptide and was also the NH2 terminus of the CNBr fragment Ly. The sequence of the tryptic peptide LO-2, which overlaps L2 and La, is also shown in Figure 1. Methionine was the NH2terminus of this overlap peptide, and CNBr cleavage produced free homoserine. The remaining hexapeptide LO-2b showed phenylalanine at the NH, terminus as did Ls. This confirms that the order of the light-chain CNBr fragments is L1-Ll-Ls. Order of the Heacy-Chuin CNBr Fragments. THE Fd(t) PORTION of the heavy chain contains the CNBr fragments H1, Hz, Ha and H ~ A (Waxdal et al., 1968). Reduced and alkylated Fd(t) was digested with trypsin and two methionine-containing tryptic peptides, HO-1 and HO-2, were isolated according to the fractionation scheme shown in Figure 2. The amino acid compositions of these two peptides are presented in Table 11. HO-1 contained two methionine residues and therefore must overlap three CNBr fragments. This arrangement is possible only if HO-1 contains a region corresponding to CNBr fragment H?. As expected, CNBr cleavage of HO-1 produced the fragment Hz (or HO-lb) in addition to two other peptides, HO-la and HO-lc (Figure 2). The partial sequence shown in Figure 3 was derived from a knowledge of the "2and COOH-terminal residues of HO-1, HO-la, HO-1 b and HO-lc. Tryptic digestion of the CNBr fragment HI yielded a COOH-terminal peptide identical in composition with HO-la (Figure 3). This established the order of the first two CNBr fragments as HI-H,. Phenylalanine was the

NHy-terminal residue of the peptide HO-IC and therefore must be the NH9 terminus of the third CNBr fragment. Of the two remaining fragments from the Fd(t) portion of the heavy chain (H3 and H4*) only H 3 possessed an NHz-terminal phenylalanine (Table I). As expected, tryptic digestion of H3yielded an NHy-terminal peptide with a composition identical with HO-lc. This finding not only establishes the order of the CNBr fragSoluble Tryptic Peptldes of Fd i t )

Gradient1 Gradient11

,

1

CNIr

,

AG-l x 2

2: Summary of the procedure for the isolation of tryptic overlap peptides HO-1 and HO-2 from the Fd(t) portion of the heavy chain (see Materials and Methods). HOAc, acetic acid. FIGURE

1969

COVALENT S T R U C T U R E OF YG-IMMUNOGLOBULIN

BIOCHEMISTRY

Overlap tryptic peptide containing HO-1 methionine Glx(Glxz,Pro,Gly,,Ala,Leu,Met,Gly.Pro,GIy,Val,lle,Met, Phe,Asx,Glx,Pro?,Gly,Ala,Tyr)Lys CNBr fragments HO- 1a HO-lb HO-lc of overlap peptides Glx(Glxz,Pro,GlyP,Ala,Leu)Hsr /Gly(Pro,Gly,Val,Ile)Hsr 1 Phe(Asx,Glx,Pro2,Gly,Ala,Tyr)Lys COOH- and NH2COOH-terminal tryptic peptide "?-terminal tryptic terminal tryptic of HI HP peptide of H1 peptides of CNBr Glx(GlxP,Pro,GlyP,Ala,Leu)Hsr/Gly(Pro,Gly,Val,Ile)Hsr(Phe(Asx,Glx,Pr~~,Gly.Ala,Tyr)Lys fragments from Fd(t) FIGURE 3 : Ordering of the CNBr fragments (HI, HP,and HB) from the Fd(t) portion of the heavy chain by comparison of their terminal tryptic peptides or amino acid residues with the tryptic overlap peptide HO-1.

Overlap tryptic peptide containing methionine CNBr fragments of overlap peptide COOH- and NHP-terminal tryptic peptides of CNBr fragments from Fd(t) FIGURE

HO-2

Val(Asx~,Thra,Ser,Glx,Alas,Ile,Tyr,Met,Glx,Serz.Leu?)Arg HO-2a

Val(Asxs,Thrr,Ser,Glx,Alan,Ile,Tyr)Hsr COOH-terminal tryptic "*-terminal peptide of H3 of Hq Val(AsxP,Thr4,Ser,G1x,Ala2,11e,Tyr)Hsr /Glu(Ser,Leu?)Arg

4: Ordering of CNBr fragments Ha and Hq of the heavy chain by comparison with tryptic overlap peptide HO-2.

ments as HI-H2-H3, but completes the ordering of the Fd(t) portion of the heavy chain. H I has already been assigned as the NH2-terminal CNBr fragment of the heavy chain from data on NH2-terminal residues (Table I, Waxdal et al., 1968). The remaining fragment from the Fd(t) region, H4A,was placed at the COOH-terminal end of the Fd(t) fragment, because H 4is the site of tryptic hydrolysis of the heavy chain during the production of Fab(t) and Fc(t) (Waxdal et af., 1968). This assignment has been confirmed by analysis of the second overlap peptide from the Fd(t) region, HO-2 (Figure 4). The amino acid composition of HO-2 is presented in Table 11. This peptide was treated with CNBr and two smaller peptides, HO-2a and HO-2b, were produced (Figures 2 and 4). Tryptic digestion of Ha yielded the COOH-terminal peptide identical in composition with HO-2a. The sum of the composition of this peptide and of the NH2-terminal peptide of Hq was equal t o the composition of HO-2. Consequently, the order of the CNBr fragments in the Fd(t) region of the heavy chain is confirmed as HI-HZ-HS-H~A. THEFc(t) PORTION of the heavy chain contained the Soluble Tryptic Peptides of Fc ( t )

AG-50x4 Gradient

I AG-50x 4 Gradient I

Oxldlzed with

CNBr fragments H ~ RHs, , He, and Hi.Because Hd is the site of tryptic hydrolysis to form Fab(t), H 4 was ~ assigned to the NHderminal position of Fc(t) (Waxdal et al., 1968). Hi was placed at the COOH terminus of the heavy chain, because this CNBr fragment contained no homoserine. With the order H,B(HI,H~)H;,it was only necessary to confirm the adjacent positions of one pair of CNBr fragments to complete the ordering of the heavy-chain fragments. Two of the three possible methionine-containing peptides were isolated from a tryptic digest of the Fc(t) fragment by means of the fractionation procedures summarized in Figure 5. The amino acid composition of overlap peptide HO-3 is presented in Table TI. When HO-3 was treated with CNBr, two smaller peptides, HO-3a and HO-3b, were produced (Figures 5 and 6). The COOH-terminal tryptic peptide of Hqhad an amino acid composition identical with HO-3a (Figure 6), and therefore the overlap peptide HO-3 must extend from H 4 to either H a or He. Both HO-3b and H 5 had isoleucine as their NH?-terminal residue (Table I, Figure 6). This observation was sufficient t o determine the order of the CNBr fragments in Fc(t) as H4~-Hj-Hg-H7. This order is consistent with the partial amino acid sequence of the final overlap peptide, HO-4 (Figure 6). The tryptic peptide was difficult to purify, and it was necessary t o oxidize the methionyl residue to the sulfone during the isolation procedure. Because oxidation made subsequent CNBr cleavage impossible, HO-4 was submitted to the dansyl-Edman procedure. The amino acid sequence around the methionyl residue was -GlxMet-Thr-. The NH, terminus of He (Table I) was threonine.

Gradient I

Discussion

1970

FIGURE 5: Summary of procedures used to isolate tryptic overlap peptides HO-3 and HO-4 from the Fc(t) portion of the heavy chain (see Materials and Methods).

WAXDAL,

KONIGSBERG,

AND

EDELMAN

The isolation and analysis of methionine-containing tryptic peptides have enabled us t o order the CNBr fragments of the yG-immunoglobulin Eu. The order and composition of the fragments and information on the

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Overlap tryptic peptide containing methionine

HO-3 HO-4 Asx-Thr-Leu-Met-Ile-Ser-Arg Thr-Leu-Pro-Pro-Ser-Arg-GIx-Glx-Met-Thr-(Ser,Glx,Lys)

CNBr fragments of overlap peptide

FIO-3a HO-3b Asx-Thr-Leu-tlsr 1 Ile-Ser-Arg

COOH- and NHs-terminal

COOH-terminal NHAerminal COOH-terminal NH2of H j terminal tryptic peptide of H j of Ha of He Asx-Thr-Leu-HsrIIle. . . , . . . . . , . . , . . . . . , . . . . . . . . . . . , . . . , . . . . . Hsr Thr. . . .

tryptic peptides of CNBr fragments from Fc(t)

6: Ordering of the CNBr fragments from the Fc(t) portion of the heavy chain by comparison of their terminal tryptic peptides or amino acid residues with the amino acid sequence of the tryptic overlap peptides HO-3 and HO-4.

FIGURE

interfragment disulfide bonds (Edelman et ul., 1968; Waxdal et al., 1968; Gall et a/., 1968) may be incorporated in a detailed model of the molecule (Figure 7). The model is composed of two identical halves, each containing ten CNBr fragments and consisting of a pair of heavy and light chains joined by a disulfide bond between the COOH-terminal residue of the light chain and the region of the heavy chain corresponding to CNBr fragment H ~ AThe . half-molecules are joined by two disulfide bonds in the heavy chains located in the region ccrresponding to fragment H ~ BThe . verification of the number and location of the interchain bonds and the determination of the amino acid sequence of the heavy chain around these bonds are presented in the next paper of this series (Gall et al., 1968). The exact positions of the disulfide bond joining H I to Ha (Figure 7) and of the carbohydrate in fragment Hs have not been established. The remainder of the disulfide bonds so far accounted for are assigned on the basis of studies of the CNBr fragments (Waxdal etaf., 1967, 1968); studies to determine their exact positions are in progress. LI and L2 are joined by a disulfide bond, and there is an intrachain disulfide bond in L3. Recent studies of the disulfide bonds of another human yG-immunoglobulin (Pink and Milstein, 1967) are consistent with these assignments. The major site where trypsin cleaves the heavy chain t o produce the enzymatic fragments Fab(t) and Fc(t) is indicated by the broken arrows (Figure 7). Both the number and the position of the methionyl residues in Eu light and heavy chains may be compared to the published data on type K Bence-Jones proteins (Hilschmann and Craig, 1965; Milstein, 1965; Titani et ai., 1965) and the heavy chain of another human yGimmunoglobulin, Daw (Press et al., 1966a,b). The partial amino acid sequences of the several type K Bence-Jones proteins show only one methionine residue at position 4 in the chain (Hilschmann and Craig, 1965; Milstein, 1965; Titani et a/., 1965). The K chain of Eu contains two other methionine residues in the variable region which are the major sites of cleavage upon CNBr treatment (Waxdal et af., 1968). The methionyl residues in the heavy chain of Eu did not correspond to those in Daw (Press et al., 1966a), with the exception of the residues linking Hd and Hs (see Gall et a/., 1968) and Hs and Hi. The COOH-terminal CNBr fragment of heavy chain, Hi, which contains 18 amino acid residues, is identical with the corresponding fragment from the heavy chain of Daw (Waxdal et ai., 1968). Pooled human yG-immunoglobulin has also been found to contain this fragment (Piggot and Press, 1966), and CNBr fragments of the same size, but differ-

ing in composition by two residues, have been isolated from the yG-immunoglobulin heavy chains of rabbit (Givol and Porter, 1965; Hill et ai., 1966b) and horse (Press et a/., 1966a). The "*-terminal CNBr fragment of the heavy chain from Eu (HI) was found to be larger than the Corresponding fragment from Daw. In both cases the fragments are linked by a disulfide bond to a large central CNBr fragment (Press er af., 1966a; Waxdal et al., 1968). Thorpe and Deutsch (1966) have reported the sequence of a peptide similar to HO-4 and have suggested that this peptide contaihs the marker for y 2 b , G m (a-) heavy chains. Although Eu has been typed as G m (a-), the partial amino acid sequence of HO-4 (Thr-Leu-ProPro-Ser-Arg-Glx-Glx-Met-Thr-, Figure 6) differs from the sequence of the peptide given by Thorpe and Deutsch (Thr-Leu-Pro-Pro-Ser-Arg-Met-Glu-Glu-ThrLys). Another human myeloma protein, He, of the same G m type as Eu, is currently being studied in our laboratory. CNBr treatment of He produces fragments apparently identical with Hs, Hs, and H7 from Eu (M. J. Waxdal and G. M. Edelmarl, unpublished results). The location of the variable region of the heavy chain of this G m type may emerge from a comparison of the CNBr fragments in the Fd region of Eu and He. The partial amino acid sequence of peptide HO-4 is similar to the sequence of the corresponding region of Tn

s-s Heavy chain

s-s

5-s

s-s

PCA

ss-s

s-SS

5-s

s-s

"2

s

s

4 I COOH

COOH

7: Linear model of the light and heavy chains of the human yG-immunoglobulin Eu. The large vertical divisions in each chain denote the positions of the methionyl residues cleaved by the CNBr treatment. The relative lengths of the lines between the vertical bars are proportional to the molecular weights of each of the CNBr fragments. The numbers under the lines identify the fragments. CHO indicates that fragment H, contains the carbohydrate group. PCA indicates the blocked NH2 terminus of the heavy chain, probably pyrrolidonecarboxylic acid. The major site of proteolysis of the heavy chain by trypsin (Tn) to produce Fab(t) and Fc(t) fragments is denoted by arrows. Assignment of the intrachain disulfide bonds is made on the basis of studies of the CNBr fragments and is provisional. The interchain bonds have been located and identified (cf. FIGURE

Gall et a / . , 1968).

1971

COVALENT STRUCTURE OF TG-IMMUNOGLOBULIN

R I

pooled rabbit Fc fragments (Hill et al., 1966b). In addition, the peptide HO-3 which overlaps Hq and H5of Eu is identical in sequence with a methionine-containing peptide from pooled rabbit Fc fragments (Hill et af., 1966b) and is found at approximately the same position as in rabbit yG-immunoglobulin (Hill et a/., 1966b). These homologies and the close resemblance of the sequences around t he heavy-chain-heavy-chain disulfide bonds (Steiner and Porter, 1967; Gall et a/., 1968) provide additional evidence for the close evolutionary relationships (Hill et d.,196623) among immunoglobulins of different species.

Acknowledgments The authors wish to acknowledge the excellent technical assistance of Mrs. Elaine Shown and Miss Catherine Volin.

References Catravas, G. N. (1964), Anal. Chem. 36,1146. Cunningham, B. A., Gottlieb, P. D., Konigsberg, W. H., and Edelman, G. M. (1968), Biochemistry 7, 1983 (this issue; paper V). Easley, C . (1965), Biochim. Biophys. Acta 107,386. Edelman, G. M. (1967), in Nobel Symposium 3 , Gamma Globulins, Structure and Control of Biosynthesis, Killander, J., Ed., Stockholm, Almqvist, and Wiksell, p 89. Edelman, G. M., Gall, W. E., Waxdal, M. J., and Konigsberg, W. H. (1968), Biochemistry 7, 1950 (thisissue; paper I). Edelman, G. M., Waxdal, M. J., Gall, W. E., and Konigsberg, W. H. (1967), VII Intern. Congr. Biochem., Tokyo, 471. Gall, W. E., Cunningham, B. A., Waxdal, M. J., Konigsberg, W. H., and Edelman, G. M. (1968), Biochemistry 7,1973 (this issue; paper IV).

1972 W A X D A L ,

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A N D E D E L M A N

o c H I: M I s ~r11 Y

Givol, D., and Porter, R. R. (1965), Biochem. J . 97,32c. Gray, W. R. (1967), Methods Enzymol. 11,139. Hill, R. L., Delaney, R., Fellows, R. E., Jr., and Lebovitz, H. E. (1966a), Proc. Natl. Acad. Sci. U. S . 56,1762. Hill, R. L., Delaney, R., Lebovitz, H. E., and Fellows, R. E., Jr. (1966b), Proc. Roj~.Soc. (London) 8166, 159. Hilschmann, N., and Craig, L. C. (1965), Proc. Nrrrl. Acad. Sci. U. S. 53,1403. Konigsberg, W. H., and Hill, R . J. (1962), J . Biol. Chem. 237,2547. Milstein, C. (1965), Nature 209,370. Piggot, P. J., and Press, E. M. (1966), Biochem. J . 99,16p. Pink, J. R. L., and Milstein, C. (1967), Nature 216, 941. Press, E. M., Givol, D., Piggot, P. J., Porter, R. R., and Wilkinson, J. M. (1966a), Proc. Roy. Soc. (London) B166,150. Press, E. M., Piggot, P. J., and Porter, R. R. (1966b), Biochem. J . 99,356. Schroeder, W. A., Jones, R. T., Cormick, J., and McCalla, K. (1962), Anal. Chem. 34, 1570. Steiner, L. A., and Porter, R . R . (1967), Biochemistry 6,3957. Thorpe, N. O., and Deutsch, H. F. (1966), Immunochemistry 3,329. Titani, K., Whitley, E., Jr., Avogardo, L., and Putnam, F. W. (1965), Science 149,1090. Waxdal, M. J., Konigsberg, W. H., and Edelman, G. M. (1967), Cold Spring Harbor Symp. Quant. B i d . 32,53. Waxdal, M. J., Konigsberg, W. H., Henley, W. L., and Edelman, G. M. (1968), Biochemistry 7, 1959 (this issue; paper 11). Woods, K. R., and Wang, K.-T. (1967), Biochim. Biophys. Acta 133,369. World Health Organization (1964), Bull. World Health Organ. 30,447.